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采用 RecA 和一种限制酶提高 HLA-DRB1 基因分型的环介导等温扩增特异性。

Improved loop-mediated isothermal amplification for HLA-DRB1 genotyping using RecA and a restriction enzyme for enhanced amplification specificity.

机构信息

Department of Molecular Life Science, Division of Basic Medical Science and Molecular Medicine, School of Medicine, Tokai University, Isehara, Kanagawa, Japan.

出版信息

Immunogenetics. 2013 Jun;65(6):405-15. doi: 10.1007/s00251-013-0690-0. Epub 2013 Mar 9.

DOI:10.1007/s00251-013-0690-0
PMID:23474534
Abstract

Our aim was to test and develop the use of loop-mediated isothermal amplification (LAMP) for HLA-DRB1 genotyping. Initially, we found that the conventional LAMP protocols produced non-specific and variable amplification results depending on the sample DNA conditions. Experiments with different concentrations of DNase in the reaction mixture with and without T4 DNA ligase-treated samples suggested that the strand displacement activity of DNA polymerase in LAMP, at least in part, started from randomly existing nicks because T4 DNA ligase treatment of sample DNA resulted in no amplification. Such non-specific amplification due to the randomly existing nicks was improved specifically by the addition of RecA of Escherichia coli and a restriction enzyme, for example, PvuII, to the reaction mixture. We applied the modified LAMP (mLAMP) (1) to detect specific HLA-DRB1 alleles by using only specific primers for amplification or (2) for genotyping in multiple samples with a multi-probe typing system. In the latter case, HLA-DRB1 genotyping was developed by combining the mLAMP with amplicon capture using polymorphic region-specific probes fixed onto the bottom of the wells of a 96-well plate and the captured amplicons visualized as a black spot at the bottom of the well. The multi-probe human leukocyte antigen (HLA) typing method and the specific HLA allele detection method could be applied for point-of-care testing due to no requirement for specific and expensive instruments.

摘要

我们的目的是测试和开发环介导的等温扩增(LAMP)用于 HLA-DRB1 基因分型的用途。最初,我们发现传统的 LAMP 方案根据样品 DNA 条件产生非特异性和可变的扩增结果。在反应混合物中含有不同浓度的 DNase 并进行 T4 DNA 连接酶处理的样品实验表明,LAMP 中 DNA 聚合酶的链置换活性至少部分地从随机存在的缺口开始,因为 T4 DNA 连接酶处理的样品 DNA 导致没有扩增。通过在反应混合物中添加大肠杆菌 RecA 和限制性内切酶(例如 PvuII),可以特异性地改善由于随机存在的缺口而导致的这种非特异性扩增。我们应用改良的 LAMP(mLAMP)(1)通过仅使用用于扩增的特异性引物来检测特定的 HLA-DRB1 等位基因,或者(2)通过多探针分型系统在多个样品中进行基因分型。在后一种情况下,通过将 mLAMP 与使用固定在 96 孔板孔底部的多态性区域特异性探针进行扩增子捕获相结合来开发 HLA-DRB1 基因分型,并且捕获的扩增子在孔的底部可视化作为黑点。由于不需要特定和昂贵的仪器,多探针人类白细胞抗原(HLA)分型方法和特定 HLA 等位基因检测方法可用于即时护理测试。

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